4.5 Article

Dual arginine recognition of LRRK2 phosphorylated Rab GTPases

BIOPHYSICAL JOURNAL (2021)

Get Full Text
Add to Collection

Journal

BIOPHYSICAL JOURNAL
Volume 120, Issue 9, Pages 1846-1855

Publisher

CELL PRESS
DOI: 10.1016/j.bpj.2021.03.030

Keywords

-

Categories

Biophysics

Funding

  1. Program for Cellular and Molecular Medicine, Boston Children's Hospital
  2. National Institute of General Medical Sciences from the National Institutes of Health [P30 GM124165]
  3. NIH-ORIP HEI grant [S10OD021527]
  4. DOE Office of Science [DE-AC0206CH11357, DE-SC0012704]
  5. UK Medical Research Council [MC_UU_12016/2]

Ask authors/readers for more resources

Protocol

Community support

Reagent

Community support

This study reveals the mechanism by which the effector protein RILPL2 recognizes phosphorylated Rab8a through a newly identified RBD motif termed X-cap, regulating ciliogenesis. The research also demonstrates the essential role of a distal arginine residue R130 in stabilizing the primary salt bridge between RILPL2 and phospho-Rab through favorable enthalpic contributions, providing insights into the assembly of phospho-Rab complexes by LRRK2 activation.
Parkinson's-disease-associated LRRK2 is a multidomain Ser/Thr kinase that phosphorylates a subset of Rab GTPases to control their effector functions. Rab GTPases are the prime regulators of membrane trafficking in eukaryotic cells. Rabs exert their biological effects by recruitment of effector proteins to subcellular compartments via their Rab-binding domain (RBD). Effectors are modular and typically contain additional domains that regulate various aspects of vesicle formation, trafficking, fusion, and organelle dynamics. The RBD of effectors is typically an a-helical coiled coil that recognizes the GTP conformation of the switch 1 and switch 2 motifs of Rabs. LRRK2 phosphorylates Rab8a at T72 (pT72) of its switch 2 a-helix. This post-translational modification enables recruitment of RILPL2, an effector that regulates ciliogenesis in model cell lines. A newly identified RBD motif of RILPL2, termed the X-cap, has been shown to recognize the phosphate via direct interactions between an arginine residue (R132) and pT72 of Rab8a. Here, we show that a second distal arginine (R130) is also essential for phospho-Rab binding by RILPL2. Through structural, biophysical, and cellular studies, we find that R130 stabilizes the primary R132:pT72 salt bridge through favorable enthalpic contributions to the binding affinity. These findings may have implications for the mechanism by which LRRK2 activation leads to assembly of phospho-Rab complexes and subsequent control of their membrane trafficking functions in cells.

Authors

I am an author on this paper
Click your name to claim this paper and add it to your profile.

Reviews

Primary Rating

4.5
Not enough ratings

Secondary Ratings

Novelty
-
Significance
-
Scientific rigor
-
Rate this paper

Recommended

No Data Available
No Data Available
Webinars Posters Questions Hubs Funding Journals Papers Connect Collections Reviewers About Us FAQs Mobile App Privacy Policy Terms of Use
© Peeref 2019-2024. All rights reserved.